Genome sequencing, assembly, and annotation of the self-flocculating microalga Scenedesmus obliquus AS-6-11

Background Scenedesmus obliquus belongs to green microalgae and is widely used in aquaculture as feed, which is also explored for lipid production and bioremediation. However, genomic studies of this microalga have been very limited. Cell self-flocculation of microalgal cells can be used as a simple and economic method for harvesting biomass, and it is of great importance to perform genome-scale studies for the self-flocculating S. obliquus strains to promote their biotechnological applications. Results We employed the Pacific Biosciences sequencing platform for sequencing the genome of the self-flocculating microalga S. obliquus AS-6-11, and used the MECAT software for de novo genome assembly. The estimated genome size of S. obliquus AS-6-11 is 172.3 Mbp with an N50 of 94,410 bp, and 31,964 protein-coding genes were identified. Gene Ontology (GO) and KEGG pathway analyses revealed 65 GO terms and 428 biosynthetic pathways. Comparing to the genome sequences of the well-studied green microalgae Chlamydomonas reinhardtii, Chlorella variabilis, Volvox carteri and Micractinium conductrix, the genome of S. obliquus AS-6-11 encodes more unique proteins, including one gene that encodes D-mannose binding lectin. Genes encoding the glycosylphosphatidylinositol (GPI)-anchored cell wall proteins, and proteins with fasciclin domains that are commonly found in cell wall proteins might be responsible for the self-flocculating phenotype, and were analyzed in detail. Four genes encoding both GPI-anchored cell wall proteins and fasciclin domain proteins are the most interesting targets for further studies. Conclusions The genome sequence of the self-flocculating microalgal S. obliquus AS-6-11 was annotated and analyzed. To our best knowledge, this is the first report on the in-depth annotation of the S. obliquus genome, and the results will facilitate functional genomic studies and metabolic engineering of this important microalga. The comparative genomic analysis here also provides new insights into the evolution of green microalgae. Furthermore, identification of the potential genes encoding self-flocculating proteins will benefit studies on the molecular mechanism underlying this phenotype for its better control and biotechnological applications as well. Supplementary information Supplementary information accompanies this paper at 10.1186/s12864-020-07142-4.


Background
Microalgae are widely studied for producing biofuels and mitigating greenhouse gas emissions [1]. In addition, microalgae are also producers of various high-value biochemicals, such as lipids, proteins, polysaccharides, pigments, vitamins, and antioxidants [2]. For economic bioproduction by microalgae, robust strains and optimized processes are both essential [3]. Genome-scale studies of microalgae can provide in-depth information on intracellular metabolism from a global prospect [4][5][6], and benefit the development of robust microalgal strains and efficient processes. Therefore, studies on genome sequencing and annotation of microalgae have received increasing attention.
Due to small cell size, negative surface charge and low biomass concentration achieved during photosynthetic autotrophic culture, harvesting microalgae biomass from a large volume of culture medium is a great challenge for their biorefinery [7,8]. Among various technologies developed for microalgal biomass recovery, gravity sedimentation facilitated by the flocculation of microalgal cells is more economically competitive [8]. On the other hand, some microalgal strains can flocculate or aggregate spontaneously [9][10][11]. The self-flocculation of microalgal cells enables their harvest without the addition of exogenous flocculants, and biomass harvesting based on the selfflocculation of microalgal cells is more environmentally friendly compared to the flocculation of microalgal cells through physical and chemical methods, or induced by infochemicals from predators [8,12].
Despite the progress in using cell flocculation of microalgae for biomass recovery, in-depth studies on mechanisms of microalgal cell flocculation are still lacking. So far, microalgal cell wall polysaccharide and other extracellular polymeric substances (EPS) containing sugars and proteins have been identified as flocculating agents [10,11,13], but genes involved in the process remain unexplored. Identification of genes involved in microalgal cell self-flocculation is of importance to develop robust strains with controlled flocculation phenotype for microalgal biorefinery, which can be enabled by the advancement of genetic engineering of microalgae [14].
Scenedesmus belongs to green microalgae and is useful for lipid and pigment production, wastewater treatment, heavy metal removal and CO 2 fixation [14][15][16][17][18]. The selfflocculating microalga S. obliquus AS-6-1 showing great advantages in microalgal cell harvest and heavy metals adsorption was reported previously [10,16]. However, genes encoding key protein(s) for the synthesis of flocculating agents in S. obliquus are still not clear. To date, the genome sequences of four Scenedesmus strains are available (NCBI BioProjects PRJNA498405, PRJNA394817, PRJNA394817 and PRJNA428298), but none of them have been annotated adequately. Three of these genomes lack annotation information, and the annotation of the remaining strain Scenedesmus sp. ARA is incomplete due to the large contig numbers of 4727 and a low N50 value of 37,561. Additionally, the three Scenedesmus genomes were sequenced by the second-generation sequencing (SGS) technology that might cause bias annotation due to shorter read lengths compared with Pacific Biosciences (Pacbio) sequencing technology [19].
In this study, we sequenced the self-flocculating S. obliquus AS-6-11 genome using the Pacbio technology and reported its genome assembly and annotation. We explored the metabolic potential of this microalga, and performed comparative genome analyses with the other four annotated microalgal genomes. We also comprehensively analyzed the cell wall proteins of S. obliquus AS-6-11 that might act as the flocculating agents for the self-flocculating phenotype. The knowledge obtained in this work can not only benefit understanding and control of the self-flocculation of microalgal cells, but will also provide insights for further genome-scale studies of S. obliquus and other related microalgae to explore their biotechnological potentials.

Morphological features and genome assembly
Cell self-flocculation of S. obliquus AS-6-11 was observed by SEM analysis. The microalgal cells are round and form aggregates through cell-cell contacts (Fig. 1), which is different from the other reported Scenedesmus strains that are in spindle shape [12].
The estimated genome size of S. obliquus AS-6-11 is 172.3 Mbp with 2772 contigs, and the N50 contig size is 94.4 kbp using MECAT for the genome assembly (Additional file 1: Table S1; NCBI BioProject ID: PRJNA593662). Results using the MECAT software showed a better assembly ability than that of SMRT Portal in S. obliquus AS-6-11, in which the contig numbers are 58.1% less, and the N50 value is 1.5-fold higher (Additional file 1: Table S1). The genome sizes of the released Scenedesmus strains [20][21][22][23][24] range from 23.4 to 208.0 Mbp (Table 1). Among the available results, the N50 contig sizes of S. obliquus AS-6-11 reported in this study and S. obliquus strain DOE0152z using Pacbio technology are significantly higher than the other Scenedesmus strains using SGS ( Table 1). The N50 contig size of S. obliquus AS-6-11 is 1.2-fold and 10.7-fold higher than Scenedesmus sp. MC-1 and S. quadricauda LWG 002611, respectively. Besides, the GC content of Scenedesmus strains ranges from 52.0 to 63.2%, and S. obliquus AS-6-11 has the lowest GC content (Table 1). Benchmarking Universal Single-Copy Orthologs (BUSCO) analysis showed that the assembly of S. obliquus AS-6-11 is 87.1% complete with 2168 BUSCO groups (Additional file 2).

Genome annotations
A total of 31,964 protein-coding genes were predicted in the S. obliquus AS-6-11 genome ( Table 2). The predicted gene number of S. obliquus AS-6-11 genome is dramatically higher than the other Scenedesmus strains (Table 1). According to the Non-redundant protein (NR), SWISS-PROT, and Pfam protein families databases, 19,847, 13,099, and 13,612 proteins were annotated, respectively ( Table 2). The protein number annotated based on the NR database is the largest, which is 1.52-fold higher than that obtained based on the SWISS-PROT database. Besides, 65 GO terms and 428 pathways were predicted by Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) databases in S. obliquus AS-6-11, respectively.
The top 20 GO terms and KEGG pathways enriched in gene function annotation of the S. obliquus AS-6-11 genome were illustrated in Fig. 2. The top 20 GO terms are mainly located in biological process (10) and cellular component (8), in which the cell, cell part, and organelle are the top three GO terms (Fig. 2a). The top 20 KEGG pathways are mainly related to genetic information processing (14), in which chromosome and associated proteins, membrane trafficking, and spliceosome are the top three KEGG pathways (Fig. 2b).

Comparative genomic analysis based on KEGG pathways
A total of 428 pathways were annotated in the S. obliquus AS-6-11 genome. In terms of lipid metabolism, the fewest genes (171) were annotated in S. obliquus AS-6-11, especially in glycerolipid metabolism, glycerophospholipid metabolism and arachidonic acid metabolism (Table 3). However, more genes related to fatty acid biosynthesis and elongation were identified in S. obliquus AS-6-11 than that in C. reinhardtii and V. carteri (Table  3). Moreover, genes in the carotenoid biosynthesis in S. obliquus AS-6-11 are the fewest.

Comparative genomic analysis of orthologous gene clusters
Comparing with the other four species, S. obliquus AS-6-11 has 15,879 gene clusters with 14,576 orthologous clusters and 1303 single-copy gene clusters (Fig. 3). There are 3357 overlapping orthologous gene clusters among the five microalgae. S. obliquus AS-6-11 has the most gene clusters and singletons (defined as the singleton genes for which no orthologs could be found in any of the other species [25]), and the number (8751) is 1.26-fold, 3.71-fold, 5.34-fold and 1.67-fold higher than that in C. reinhardtii, C. variabilis, M. conductrix and V. carteri, respectively (Fig. 3). Comparative orthologous gene cluster analysis also showed that the phylogenetic  proximity of S. obliquus AS-6-11 is very similar to that of the other four microalgae (Additional file 3: Fig. S1).

Comparative genomic analysis based on gene families
A total of 3608 gene families were identified in S. obliquus AS-6-11, in which 136 unique gene families existed (Fig. 4). Both the total and unique gene families in S.

Analysis of the genome features related to cell selfflocculation
Cell self-flocculation of budding yeast Saccharomyces cerevisiae has been well-studied. The flocculation proteins, for example, Flo1p, Flo5p, Flo9p, and Flo10p, are cell wall proteins (CWPs) and also called lectin [26,27]. GPI-anchor was reported as the common element in cell adhesion proteins and the GPI-anchored adhesins in yeast species of Candida albicans and S. cerevisiae are the well-known fungal adhesions [28]. In S. obliquus AS-6-11, a total of 432 GPI-anchored CWPs are identified. Analysis of the top 10 GPI-anchored CWPs indicated that seven of them has the transmembrane region, and eight of them had the signal peptides ( Table 4). The isoelectric point (pI) and molecular weight (Mw) of the GPI-anchored CWPs vary from 4.95 to 9.58 and 6.10 KDa to 78.84 KDa, respectively (Table 4).
Fasciclin (PF02469) is an extracellular domain (http:// pfam.xfam.org/family/PF02469) that belongs to the ancient cell adhesion domain that is common to plants and animals. So far, fasciclin domain proteins have not been analyzed in microalgae. In the S. obliquus AS-6-11 genome, a total of 33 fasciclin domain proteins are identified, which are divided into three groups (Fig. 5a). Three main motifs are randomly distributed across the fasciclin domain proteins (Fig. 5b). The predicted pI values and Mw greatly differ among the fasciclin domain proteins (Additional file 4: Table S2). The subcellular localization prediction of fasciclin domain proteins indicated that most proteins have cytoplasmic (cyto) sites, and 15 of them have secreted (extr) sites (Additional file 4: Table S2). Further analysis of these 15 fasciclin domain proteins containing extr sites showed that six proteins are homologous to the reported fasciclin proteins of Monoraphidium neglectum (64.84%), Aquabacterium sp. (61.36%), Scenedesmus sp. Ki4 (48.09%), Pelomonas puraquae (46.94%) ( Table 5). Additionally, two of the predicted proteins are annotated into the extracellular region part according to the GO database.
Combining analysis of GPI-anchored CWPs and fasciclin domain proteins, four fasciclin domain proteins were found to distribute in GPI-anchored CWPs ( Fig. 6a; Additional file 5), in which one has two FAS1 domains (four repeated domains in the fasciclin I family of proteins), two have transmembrane regions, and one has signal peptide (Fig. 6a). Comparative genomic analysis of S. obliquus AS-6-11 and the other four microalgae species (C. reinhardtii, C. variabilis, M. conductrix and V. carteri) revealed no similar proteins to the four fasciclin domain proteins. We also performed comparative transcriptome analysis of S. obliquus AS-6-11 and the nonflocculating S. obliquus FSP-3, and the results showed that the four fasciclin domain protein-encoding genes (Fig. 6a) had transcription level in S. obliquus AS-6-11, but the transcription of these genes cannot be detected in S. obliquus FSP-3 (Additional file 6: Table S3).
The unique gene family D-mannose binding lectin was also analyzed (Additional file 5). One gene belongs to this unique gene family was identified, and the encoded protein has two conserved domains: CAP (cysteine-rich secretory proteins) domain and B_lectin (D-mannose binding lectin) domain. The putative D-mannose binding lectin of S. obliquus AS-6-11 is homologous to a secreted glycoprotein Pry1p of S. cerevisiae YJM693 (SGD ID: S000003615), and the identity is 58% (Fig. 6b). The similarity between Pry1p and D-mannose binding lectin attributes to the same CAP domain (Fig. 6b).

Discussion
Genome feature of S. obliquus AS-6-11 We report here the genome sequence and annotation of S. obliquus AS-6-11, which is the first sequenced selfflocculating microalgal genome, and is also so far the most comprehensively annotated genome among the available S. obliquus genome information. The much larger gene numbers of S. obliquus AS-6-11 (Table 1) suggested its unique feature. Considering the relative completeness of S. obliquus AS-6-11 genome and the lack of S. obliquus genome annotation, S. obliquus AS-6-11 may serve as a model alga for supplying reference genome annotation and investigating the gene function, evolution, and biotechnology application of S. obliquus strains.
We obtained a larger contig N50 size of S. obliquus AS-6-11 genome than that of Scenedesmus sp. MCand S. quadricauda, which may attribute to Pacbio sequencing technology and the assembly tool MECAT [29]. The MECAT software showed higher computing Fig. 3 The orthologous gene clusters in the five microalgae. a. The shared and different orthologous gene clusters; b. The size of each orthologous gene clusters efficiency with comparable or improved genome results than other current tools for de novo assembly of large genomes [29], and this study is the first application of this tool in the genome assembly of microalgae.
Comparative analysis of S. obliquus AS-6-11 genome with the other microalgae Due to the lack of genome annotations of Scenedesmus strains, we compared the S. obliquus AS-6-11 genome with four represented green microalgae ( Fig. 3; Fig. 4;      Table 3). S. obliquus AS-6-11 has more singletons, unique gene families as well as additional KEGG pathways than the other four microalgae, revealing its special evolutionary status, genomic complexity, and metabolic characteristics. Comparative genomics analysis of orthologous clusters among multiple species is important for identifying the overlap among orthologous clusters that helps to elucidate the evolution and function of proteins [25]. The similar phylogenetic proximity of S. obliquus AS-6-11 to the four green microalgae further supports that this species locates in the intermediate stage of green algae evolution [30]. Due to the potential applications of Scenedesmus strains in wastewater treatment and lipid production [31,32], their lipid metabolism needs to be well-studied. S. obliquus AS-6-11 has fewer genes of lipid metabolism compared to S. quadricauda LWG002611 and the other four green microalgae, suggesting the difference of lipid biosynthesis or genome integrity among the strains. For example, the fewer genes of arachidonic acid metabolism in S. obliquus AS-6-11 may attribute to multiple genes encoding one enzyme in other microalgae (Table 3). Key enzymes involved in triacylglycerol (TAG) biosynthesis pathways and carbon fixation were identified based on the genome sequence of S. quadricauda LWG002611, providing targets for genetic and metabolic engineering to improve biofuel production and reconstruct the metabolic pathways of this strain [22]. In the previous work, overexpression of type 2 diacylglycerol acyltransferase gene (DGTT1) of C. reinhardtii in S. obliquus CPC2 enhanced its lipid content by nearly two-fold [33]. Overexpression of acetyl-CoA carboxylase gene in Scenedesmus sp. MC-1 increased its intracellular lipid by 28.6%, indicating its importance in the lipid metabolism of Scenedesmus [21]. However, the endogenous genes involved in lipid biosynthesis in S. obliquus has not been investigated. The identified lipid biosynthetic genes in this work will facilitate improving lipid production in S. obliquus.
On the other hand, Scenedesmus can produce important pigments carotenoids as valuable products, and overexpression of synthetic phytoene synthase gene (PSY) in Scenedesmus sp. CPC2 increased β-carotene production to 30 mg g − 1 -cell [34]. So far no studies have been focused on the innate carotenoid biosynthetic genes in S. obliquus. Further investigation of the functional genome of Scenedesmus will benefit the metabolic engineering of this important microalga for carotenoids production.

Potential flocculation proteins in S. obliquus AS-6-11
Although bioflocculation has been widely accepted as a promising way to harvest microalgal biomass, studies on cell self-flocculation of microalgae are still very limited. In the previous study, cell wall polysaccharides were revealed to act as flocculating agents in S. obliquus AS-6-1 [10]. In the recent study, we found that protease treatment led to the de-flocculation of S. obliquus AS-6-11 (data not shown), indicating their different mechanisms of cell selfflocculation. Therefore, we focused on the identification of flocculating proteins in S. obliquus AS-6-11.
Yeast cell flocculation has been widely used in the beer industry and biofuels production as a simple, economic and environmentally friendly way to harvest cells [35,36]. The interaction of lectin-like receptors with adjacent mannose side chains in cell walls played a vital role in yeast flocculation [37]. In addition to lectin-glycan interaction, glycan-glycan interactions also act a pivotal part in cell-cell adhesion, and the flocculation mechanism contributes to the self-interaction of Flo proteins in the coordination of Ca 2+ [38]. In our recent studies, mechanisms of cell flocculation in an ethanol-producing bacterium Zymomonas mobilis were also revealed, where cellulose was found to be important for the cell flocculation [39]. Moreover, our previous studies [10,11] found that cell wall polysaccharides play key roles in microalgal cell self-flocculation. Considering that mannose-specific lectin plays an important role in yeast flocculation [40], the D-mannose binding lectin family gene found in the S. obliquus AS-6-11 genome may be related to cell flocculation. However, we did not find the transcription of this gene in the transcriptome data of S. obliquus AS-6-11. In the water surface-floating microalga Chlorococcum sp. FFG039, one protein in the unique gene family (jacalin-like lectin domain, PF01419) was assumed to be related to biofilm formation with the help of the lectin domain [41]. However, the gene encoding jacalin-like lectin domain protein was not found in the S. obliquus AS-6-11 genome, suggesting the different mechanisms of microalgal flocculation.
GPI-anchored proteins are widespread in eukaryotes for anchoring proteins to the extracellular surface of the plasma membrane, and are involved in multiple cellular functions [42]. GPI-anchored CWP Flo1p in S. cerevisiae is the main flocculation protein, and the GPI-anchor is necessary for Flo1p to attach to the cell wall [27]. However, the GPI-anchored CWPs in microalgae have not been analyzed. Therefore, the genome-scale analysis of GPI-anchored CWPs is of great importance. In the genome of the model plant Arabidopsis thaliana, 210 GPIanchored proteins were identified, and most of these proteins were involved in the primary modification for targeting specific proteins to the cell surface for extracellular matrix remodeling and signaling [43]. According to the GPI-anchor studies of S. cerevisiae and Arabidopsis, the identified cell wall proteins with GPI-anchor of S. obliquus AS-6-11 may be related to the attachment of proteins to the cell wall, and the potential flocculation proteins may be members among them.
Fasciclin 1 (FAS1) domain is an ancient motif in extracellular proteins widely exists in all kingdoms of life, and FAS1 proteins mediated the interactions between the cell surface and cell exterior [44]. FAS1 domain protein of V. carteri that is homology to Drosophila fasciclin I was identified as the cell adhesion protein [45], and it also caused unicells of C. reinhardtii to flocculate [46]. Therefore, the four proteins identified in this study (Fig.  6a), which are homologous to fasciclin domaincontaining proteins of Synechocystis, D. melanogaster and Galdieria sulphuraria or hypothetical protein of M. neglectum and C. variabilis, are the most likely flocculation proteins. Although we have made great efforts to investigate the potential flocculating gene function by gene disruption, the genetic transformation method of S. obliquus AS-6-11 was not successful. Alternatively, the protein-encoding genes can also be tested in various microalgal species, which will be focused in future studies. It needs to point out that in addition to the function of cell adhesion and/or flocculation, the fasciclin domain proteins in microalgae also take parts in stress response and cell wall formation. The gene encoding one fasciclin domain protein (carotenoprotein) in microalga Ki-4 was overexpressed under salt, dehydration and high light stresses, showing its function in protecting cells against photooxidative stresses [47]. In addition, the fasciclinlike arabinogalactan protein family in higher plant Eucalyptus grandis took parts in the growth and properties of the secondary cell wall [48]. To the best of our knowledge, this is the first report on the analysis of fascilin domain proteins in microalgae. It will be interesting to further explore the functions of this category of proteins. The in-depth analysis of S. obliquus AS-6-11 genome can also provide a basis for functional genomic studies of other microalgae.

Conclusions
We present here the genome sequencing, annotation, and analysis of the self-flocculating microalga S. obliquus AS-6-11. Comparative genomic analysis between S. obliquus AS-6-11 and the other microalgae reveals its strain specificities, evolutionary status as well as metabolic characteristics. Through the analysis of the protein family, the GPI-anchored CWPs and fasciclin domain proteins were identified for the first time in microalgae, and four GPI-anchored CWPs with fasciclin domain are the most potential flocculation proteins for further studies. Taken together, the draft genome of S. obliquus AS-6-11 will provide a reliable reference for the microalgae genome studies, increasing the understanding of microalgal self-flocculation mechanisms for promoting the microalgal harvest, and benefit efficiency biorefinery using microalgae.

Microalgal strain and culture conditions
The self-flocculating S. obliquus AS-6-11 was isolated from the freshwater pond in the campus of National Cheng Kung University (22°99′74.29″N, 120°22′22.30″ E) in southern Taiwan, and was preserved at National Cheng Kung University. Cells were cultured at 25°C in BG11 medium with continuous illumination of 75 μmol m 2 s − 1 and continuous air aeration.

Morphological observation
The cell shape and surface morphology of S. obliquus AS-6-11 cells were observed by scanning electron microscope (SEM, Hitachi S-3400 N II). For SEM, cells during the exponential growth phase were harvested and fixed in 2.5% glutaraldehyde solution overnight. After that, the samples were washed two times using PBS buffer (10 mM, pH 7.4), dehydrated in different concentrations of ethanol solutions, and then referred to the method of Salim et al. [49].

Genome DNA preparation and quality assessment
Two hundred milliliter cells at the exponential growth phase (Day 6) were harvested. The genome DNA of S. obliquus AS-6-11 was extracted by EZ-10 Spin Column Plant Genomic DNA Purification Kit (NO. B518261, Sangon Biotech (Shanghai) Co., Ltd.). The DNA quality was monitored and controlled by Nanodrop (Thermo Scientific NanoDrop 2000) and DNA gel electrophoresis.

Genome sequencing and assembly
The obtained high-quality DNA was sequenced using the PacBio RS II System. The size of DNA libraries was 10-20 kb and 10 SMRT cells were sequenced. Filtered Pacbio subreads were de novo assembled by software MECAT [29] and SMRT Portal with recommending parameters, respectively. Genome assembly quality using MECAT was further assessed by BUSCO (3.0.2) [50]. The following analyses were based on the MECAT assembly result.
For transcriptome analysis, S. obliquus AS-6-11 and S. obliquus FSP-3 cells grown for 48 h under the same condition were harvested at 6000 rpm for 5 min, and then washed three times with the sterilized water. The washed cells were stored at − 80°C immediately and send to Novogene Co., Ltd. for initial sequencing and analysis.

Prediction of GPI-anchored cell wall proteins
GPI-anchored CWPs in S. obliquus AS-6-11 were predicted by the GPI-anchored protein predictor developed by the National Science and technology development agency of Thailand [56]. The top 10 of predicted GPIanchored CWPs with signal peptide were further analyzed using compute pI/Mw tools of ExPASy (https:// web.expasy.org/compute_pi/) and SMART (http://smart. embl-heidelberg.de/). Protein subcellular localization sites were estimated by Protein Subcellular Localization Prediction (https://wolfpsort.hgc.jp/).

Analysis of fasciclin domain proteins
The fasciclin domain family proteins were extracted from protein family annotation files and further analyzed using compute pI/Mw tool of ExPASy, SMART, and Protein Subcellular Localization Prediction.

Phylogenetic analysis of fasciclin domain proteins
A phylogenetic tree of fasciclin domain proteins was constructed using MEGA 7 [57]. The sequence alignment was performed using MUSCLE and the phylogenetic tree was constructed using the Maximum likelihood method with 1000 bootstrap replicates.

Analysis of the conserved motifs of fasciclin domain proteins
The motifs' analysis of fasciclin domain proteins was performed by the online MEME website (http://memesuite.org/tools/meme) with the default parameters.